Micro-rheological behaviour and nonlinear rheology of networks assembled from polysaccharides from the plant cell wall

Vincent, Romaric R. R., Mansel, Brad W., Kramer, Andrea, Kroy, Klaus, Williams, Martin Alexander Keith

02 August 2022

The same fundamental questions that have driven enquiry into cytoskeletal mechanics can be asked of the considerably less-studied, yet arguably just as important, biopolymer matrix in the plant cell wall. In this case, it is well-known that polysaccharides, rather than filamentous and tubular protein assemblies, play a major role in satisfying the mechanical requirements of a successful cell wall, but developing a clear structure–function understanding has been exacerbated by the familiar issue of biological complexity. Herein, in the spirit of the mesoscopic approaches that have proved so illuminating in the study of cytoskeletal networks, the linear microrheological and strain-stiffening responses of biopolymeric networks reconstituted from pectin, a crucial cell wall polysaccharide, are examined. These are found to be well-captured by the glassy worm-like chain (GWLC) model of self-assembled semi-flexible filaments. Strikingly, the nonlinear mechanical response of these pectin networks is found

info:eu-repo/classification/ddc/530

ddc:530

Mechanical Properties of Plant Cell Wall Mimics Determined using Strain-Induced Buckling Methods / Mechanical Properties of Plant Cell Wall Mimics

Stimpson, Taylor

January 2020

A thesis submitted to the School of Graduate Studies in partial fulfilment of the requirements of the Master of Applied Science degree / This thesis investigated structure-function relationships of materials designed to mimic the plant cell wall by comparing their mechanical properties measured using strain-induced buckling methods. The plant cell wall mimics are submicrometer-thick films composed of cellulose nanocrystals (CNCs) and various types of xyloglucan (XG), a common plant hemicellulose. Our goal was to establish links between film composition/architecture and elastic modulus, to better understand the interactions between plant cell wall components and their influence on mechanical properties. Three buckling methods for measuring mechanical properties of supported films were compared. All methods involved compressing a thin film deposited onto a shape memory polymer or an elastomeric substrate, through thermal shrinking or mechanical compression, respectively. Two thermal shrinking methods (constrained in one axis or unconstrained) and one compression method (using a mechanical strain stage) were used. Based on the mismatch of mechanical properties between the film and the substrate, the rigid thin film “buckles” upon compression to dissipate strain. The resulting surface wrinkle sizes are characteristic of the mechanical properties of the thin film. A Fourier analysis algorithm with Gaussian curve fitting was optimized to extract wrinkle sizes accurately and reproducibly from microscopy images to reliably quantify the elastic moduli of thin films. To select the most precise strain-induced buckling method, model layer-by-layer (LbL) thin films composed of CNCs and polyethylene imine were tested. All three buckling methods precisely quantified the elastic moduli of the films and helped us build connections between the mechanical properties and the film composition. Elastic moduli determined were 15-44 GPa (depending on composition) and films up to 350 nm-thick were tested. Based on sensitivity analyses, however, unconstrained thermal shrinking proved to be the most robust method for calculating the elastic modulus. We believe these buckling methods may find widespread use in the characterization and surface structuring of thin films for applications in biosensors, flexible electronics, point-of-care diagnostics, and for studying plant cell wall mimics. Using the unconstrained thermal shrinking method, plant cell wall mimics were constructed using LbL thin film assembly with various concentrations of CNCs and XG. Three types of XG were compared: (1) unmodified XG, (2) XG with a fraction of the galactosyl residues removed (degalactosylated), and (3) a fragmented lower molecular weight XG. It was inferred that molecular weight impacts the stiffness of XG-CNC based on adsorption conformation of XG onto CNCs, where lower molecular weight XG results in a higher modulus film (27 ± 1 vs. 19 ± 2 GPa). As well, saccharide residues of XG, specifically galactosyl, impact XG’s capacity for self-association and interaction with CNCs, because saccharide residues hinder association through their glucan backbone. This is evidenced by the higher elastic moduli calculated for degalactosylated XG-CNC films (75 ± 6, GPa), compared to native XG-CNC films (19 ± 2 GPa). This work highlights the importance of material structure as it relates to overall performance and therefore function in natural systems, such as the plant cell wall. These studies contribute to a greater understanding of the mechanical properties of the plant cell wall and serve as a basis to extend bio-based and biomimetic materials to applications such as drug delivery, packaging, and coatings. / Thesis / Master of Applied Science (MASc) / The plant cell wall boasts impressive mechanical properties, balancing seemingly opposing properties of structural strength with flexibility. These natural materials have been a source of inspiration for new material design, but the phenomena that govern interactions between components and how their structures translate into function, have yet to be fully understood. In this work, we have constructed thin multilayered films to mimic the plant cell wall, composed of cellulose nanocrystals (rod-shaped nanoparticles derived from plant cellulose) and xyloglucan (a common hemicellulose “glue”). When the films on flexible supports are compressed, they buckle into wrinkled surface patterns that can be used to calculate their mechanical properties. This investigation compares three buckling methods and supports the notion that the mechanical performance of the plant cell wall is strongly dependent on the structure of the different components and the way they interact.

xyloglucan

cellulose

plant cell wall

elastic modulus

Fourier analysis

Characterization of lignin deposition in <i>Pinus taeda</i> L. cell suspension cultures

Eberhardt, Thomas Leonard

28 July 2008

<i>Pinus taeda</i> L. suspension culture cells were used to develop a model system to study the process of lignification occurring during the early stages of cell wall formation and maturation. Chemical, biochemical and histochemical analyses of the <i>P. taeda</i> suspension cultures grown with 2,4-dichlorophenoxyacetic acid (2,4-D) as the growth regulator did not provide conclusive evidence for lignin deposition. On the other hand, cultures in which 2,4-D was substituted with α-naphthaleneacetic acid (NAA) were shown to lignify. During this induction of lignification, limited cell wall thickening occurred since transmission electron microscopy of the 2,4-D grown cells showed only primary walls while the average cell wall thickness of the NAA-grown cells was consistent with secondary (S₁) layer formation. Despite the possibility of only limited lignin deposition in the 2,4-0 grown cells, secondary metabolism had occurred as evidenced by reversed-phase and chiral chromatographic separations which revealed the ability of these cells to produce enantiomerically pure (-)-matairesinol. Administrations of [1-¹³C], [2-¹³C ] and [3-¹³C ] specifically labeled phenylalanines to the <i>P. taeda</i> suspension cultures in medium containing NAA allowed the determination of lignin bonding patterns <i>in situ</i> by solid-state ¹³C NMR spectroscopy of the resulting ¹³C enriched cells. Aqueous and organic solvent extractions and protease treatment yielded ¹³C enriched cell walls for solid-state ¹³C NMR spectroscopic analyses of the cell wall bound lignin component. Subsequently, an isolated lignin derivative from these cell walls was analyzed by solution-state ¹³C NMR spectroscopy and verified the assignments made in the solid-state. Accordingly, the above experiments represent the first demonstration of lignin bonding patterns <i>in situ</i> in a <i>Pinus</i> species as well as a suspension culture. This culture system possesses great potential as a model to thoroughly study the early stages of lignification. / Ph. D.

LD5655.V856 1992.E237

Cell suspensions

Lignin

Loblolly pine

Plant cell walls

Characterizing RNA translocation in the parasitic weed Cuscuta pentagona

LeBlanc, Megan Leanne

03 June 2013

The obligate stem parasite Cuscuta pentagona is able to take up host plant mRNA through a specialized organ known as the haustorium. Direct cell-to-cell symplastic connections between two different organisms are rare, and the translocation mechanisms and fate of these RNAs in the parasite is not understood. To characterize this phenomenon, mobile Arabidopsis and tomato mRNAs were identified from microarray and transcriptome sequencing projects and quantified in the host-parasite system. Mobile RNAs were quantified using real time (qRT)-PCR and were found to vary substantially in their rate of uptake and distribution in the parasite. Transcripts of tomato Gibberellic Acid Insensitive (SlGAI) and Cathepsin D Protease Inhibitor (SlPI) can be traced over 30-cm of parasite stem. SlPI was abundant in the C. pentagona stem, but the number of copies decreased substantially within the first eight hours post detachment. Additional studies of mobile RNAs from Arabidopsis, Translationally Controlled Tumor Protein (AtTCTP), Auxin Response Factor (AtARF) and a Salt-inducible Zinc Finger Protein (AtSZFP) supported the idea that mRNA molecules differ in their mechanisms of uptake and mobility between host and parasite. Known phloem-mobile RNAs (SlGAI and AtTCTP) have uptake patterns that differ from each other as well as from other RNAs that are not reported to be phloem mobile (SlPI and AtSZF1). The function of RNAs in plants extend beyond protein translation to include post transcriptional gene silencing or long distance signaling, and mobile RNA in C. pentagona systems offers novel insights into this aspect of plant biology. Studies of cell-to-cell trafficking of RNAs and other macromolecules would be facilitated by the ability to manipulate individual cells. To this end, work was initiated to explore alternative approaches to understanding single cell biology using laser-mediated approaches. Optoperforation, or the use of multiphoton processes to form quasi-free electron plasmas to initiate transient pore formation in plasma membranes, has been demonstrated, but not in cells of an intact plant. This work details a protocol for optoperforation of Arabidopsis epidermal cells to allow for uptake of external dye-labeled dextrans and retention for up to 72 hours, and has the potential for transformation and molecular tagging applications. / Ph. D.

plant parasitism

Cuscuta pentagona

mRNA trafficking

optoperforation

laser-mediated plant cell disruption

host-parasite relations

<b>INVESTIGATING THE KAI2-MEDIATED SIGNALING PATHWAY OF VOLATILE SESQUITERPENES</b>

Shannon A. Stirling (18396129)

17 April 2024

<p dir="ltr">Plants emit an amazing diversity of volatile organic compounds (VOCs) that in addition to being utilized by humans for a multitude of applications, allow plants to communicate with their environment, and play numerous roles in plant growth and development. Plants must be able to perceive and distinguish between VOC cues mediating plant-plant, plant-insect, and plant-microbe interactions to appropriately respond to stimuli. Due to the plethora of biological processes dependent on VOCs, significant progress has been made towards understanding the biosynthesis of plant VOCs and their regulation, and, in recent years, the molecular mechanisms involved in VOC emission. However, to date, little is known about how VOCs are perceived by plants and trigger cellular response(s). In animals, VOCs are recognized by odorant receptors known as G-protein-coupled receptor (GPCR) proteins. However, the few GPCR genes identified in plants appear to have different functions and the lack of a reliable marker for VOC perception has hampered research in this field.</p><p dir="ltr">The discovery of natural fumigation of terpenoids in petunias provides a means of studying VOC perception and the downstream signaling pathways by providing a visual indicator of perception. Transcriptomic analysis of wild-type and transgenic petunias deficient in terpenoid synthesis revealed a link between terpene perception in pistils with the karrikin-like signaling pathway. By utilizing biochemical, computational, and in planta experiments, we demonstrate that of the four petunia karrikin-insensitive receptors (PhKAI2), one of the Lamiid-specific KAI2 intermediate clade receptors, PhKAI2ia, can stereo-specifically perceive the (−)-germacrene D signal emitted from the floral tubes, triggering a KAI2-mediated signaling cascade and affecting plant fitness. Downregulation of PhKAI2ia results in significantly smaller stigmas compared to wild-type, and the phenotype cannot be complemented by the treatment of pistils with (−)-germacrene D, indicating that PhKAI2ia transgenic plants are acting as deaf receptors. We also show that the binding of (−)-germacrene D to PhKAI2ia is sufficient to induce complex formation with more axillary growth 2 (PhMAX2) and the subsequent degradation of suppressor of MAX2 (PhSMAX1a).</p><p dir="ltr">Altogether, our research uncovers the role(s) of the intermediate clade of KAI2 receptors, illuminates the involvement of a KAI2ia-dependent signaling pathway in volatile communication, and provides new insights into plant olfaction and the long-standing question about the nature of potential endogenous KAI2 ligand(s).</p>

Plant biochemistry

Plant cell and molecular biology

KAI2

sesquiterpene

volatile plant compounds

Development of a liquid-liquid extraction method of resveratrol from cell culture media using solubility parameters

Al balkhi, M.H., Mohammad, Mohammad A., Tisserant, L-P., Boitel-Conti, M.

2016 June 1923

Yes / The extraction of bioactive compounds, produced by plant cell cultures, directly from their culture medium, which contains other by-products, is a great challenge. Resveratrol extraction from its grapevine cell cultures is considered here as an example to improve the extraction processes from plant cell cultures using solubility parameters. Successive liquid-liquid extraction (LLE) processes were exploited to extract resveratrol from the culture medium with an extraction ratio approaching 100%, high selectivity and minimum amounts of solvents. The calculations of partition coefficients as a function of solubility parameters demonstrated that benzyl benzoate is the most suitable intermediate solvent to extract resveratrol from its aqueous medium. The calculations also illustrated the high ability of methanol and ethanol to extract resveratrol from benzyl benzoate. The physicochemical properties of benzyl benzoate and processing conditions were exploited to separate it from aqueous media and organic solvents. The agitation method, component ratios and extraction time were studied to maximize the extraction yield. Under the best studied conditions, the recovery of resveratrol from different culture media approached ∼100% with a selectivity of ∼92%. Ultimately, the improved extraction processes of resveratrol are markedly efficient, selective, rapid and economical. / Mohammad Amin Mohammad gratefully acknowledges CARA (The Council for At-Risk Academics, Stephen Wordsworth and Ryan Mundy) for providing the financial support for an academic fellowship.

Benzyl benzoate

Liquid-liquid extraction

Partition coefficient

Plant cell culture

Resveratrol

Solubility parameters

Solvent consumption

Impact of UV light on the plant cell wall, methane emissions and ROS production

Messenger, David James

January 2009

This study presents the first attempt to combine the fields of ultraviolet (UV) photobiology, plant cell wall biochemistry, aerobic methane production and reactive oxygen species (ROS) mechanisms to investigate the effect of UV radiation on vegetation foliage. Following reports of a 17% increase in decomposition rates in oak (Quercus robur) due to increased UV, which were later ascribed to changes in cell wall carbohydrate extractability, this study investigated the effects of decreased UV levels on ash (Fraxinus excelsior), a fast-growing deciduous tree species. A field experiment was set up in Surrey, UK, with ash seedlings growing under polytunnels made of plastics chosen for the selective transmission of either all UV wavelengths, UV-A only, or no UV. In a subsequent field decomposition experiment on end-of-season leaves, a significant increase of 10% in decomposition rate was found after one year due to removal of UV-B. However, no significant changes in cell wall composition were found, and a sequential extraction of carbohydrate with different extractants suggested no effects of the UV treatments on cell wall structure. Meanwhile, the first observations of aerobic production of methane from vegetation were reported. Pectin, a key cell wall polysaccharide, was identified as a putative source of methane, but no mechanism was suggested for this production. This study therefore tested the effect of UV irradiation on methane emissions from pectin. A linear response of methane emissions against UV irradiation was found. UV-irradiation of de-esterified pectin produced no methane, demonstrating esters (probably methyl esters) to be the source of the observed methane. Addition of ROS-scavengers significantly decreased emissions from pectin, while addition of ROS without UV produced large quantities of methane. Therefore, this study proposes that UV light is generating ROS which are then attacking methyl esters to create methane. The study also demonstrates that this mechanism has the potential to generate several types of methyl halides. These findings may have implications for the global methane budget. In an attempt to demonstrate ROS generation in vivo by UV irradiation, radio-labelling techniques were developed to detect the presence of oxo groups, a product of carbohydrate attack by ROS. Using NaB3H4, the polysaccharides of ash leaflets from the field experiment were radio-labelled, but did not show any significant decrease in oxo groups due to UV treatments. However, UV-irradiation of lettuce leaves showed a significant increase in radio-labelling, suggesting increased UV irradiation caused an increase in the production of ROS. The study shows that the use of this radio-labelling technique has the potential to detect changes in ROS production due to changes in UV levels and could be used to demonstrate a link between ROS levels and methane emissions.

571.2

In-vitro propagation studies of the endangered succulents Drosanthemum Micans and Drosanthemum Hallii (Aizoaceae)

Mlungwana, Asanda

January 2018

Thesis (MTech (Horticulture))--Cape Peninsula University of Technology, 2018. / Drosanthemum micans and Drosanthemum hallii are endangered succulent shrubs of horticultural and medicinal value. They are restricted to the Succulent Karroo, which is one of the world’s biodiversity hotspots. The species risk extinction from illegal over-harvesting for water-wise gardens, erosion by occasional flush floods from ephemeral rivers, competition from alien invasive species, overgrazing and clearing of land for agriculture and human settlement. Although seeds and cuttings may be used in propagating these species, they often require seasonal collection and planting and cuttings struggle to establish, hence the need for in-vitro propagation as an alternative solution. Thus, the main objective of the study was to develop a method for rapid in-vitro shoot and root multiplication and acclimatization of D. micans and D. hallii. To initiate shoot formation, disinfected leaf and stem nodal explants were cultured in Murashige and Skoog (1962) media supplemented with different rates (0, 10, 20 or 30μM) of 2-isopentyladenine, 6-Benzyladenine and kinetin for D. hallii or 2-isopentyladenine, 6-Benzyladenine and Thiadiazuron for D. micans. Shoots from explants were rooted in varying rates (0, 10, 20 or 30μM) of IAA for root initiation. Three media, which were used in previous studies, were tested for acclimatization of rooted explants in i) vermiculite, ii) sand (50%): vermiculite (50%) or iii) sand (75%): perlite (25%). For quantitative evaluation of plant stress, chlorophyll fluorescence index (Fv/Fm) was measured as a proxy for plant stressf stress. It emerged that stem nodal explants of D. hallii tend to produce multiple shoots whilst leaf explants tended to produce callus when cultured in full-strength Murashige and Skoog (1962). Shoot multiplication was optimal in both D. hallii and D. micans at 10 μM of kinetin. Root formation in both D. hallii and D. micans only occurred when shoots were transferred to a full-strength Murashige and Skoog (1962) media without any phytohormones added. The intensity of tissue browning increased at higher levels of cytokinins, suggesting an interaction of plant growth regulators with exudates from explants. Different acclimatization media tested showed no significant differences in the level of stress (Fv/Fm). It is recommended that Murashige and Skoog (1962) media with10 μM kinetin be used for shoot development and multiplication, followed by transfer of the shoots to fresh full-strength Murashige and Skoog (1962) media without hormones for root development. Acclimatization of the rooted explants was possible in one of the following media: i) vermiculite, ii) sand (50%): vermiculite (50%) or iii) sand (75%): perlite (25%) and in a misted greenhouse (ca. 60% RH), with gradual weekly reductions in humidity by 10% over 2 weeks.

Drosanthemum micans

Drosanthemum hallii

Aizoaceae -- Micropropagation

Plant micropropagation

Plant tissue culture

Plant cell culture

Plants -- Analysis

Plant conservation

Expression and characterization of a human lysosomal enzyme α-iduronidase in tobacco BY-2 cells. / Expression & characterization of a human lysosomal enzyme α-iduronidase in tobacco BY-2 cells / Expression and characterization of a human lysosomal enzyme alpha-iduronidase in tobacco BY-2 cells

January 2006

Fu Lai Hong. / Thesis (M.Phil.)--Chinese University of Hong Kong, 2006. / Includes bibliographical references (leaves 106-110). / Abstracts in English and Chinese. / Thesis/Assessment Committee --- p.ii / Statement --- p.iii / Acknowledgements --- p.iv / Abstract --- p.v / 摘要 --- p.vi / Lists of Figures --- p.x / Lists of Tables --- p.xiii / List of Abbreviations --- p.xiv / Amino acid abbreviation --- p.xvi / Chapter Chapter 1 --- General Introduction --- p.1 / Chapter 1.1 --- Human α-L-iduronidase (hIDUA) --- p.2 / Chapter 1.1.1 --- Lysosomal storage disease --- p.2 / Chapter 1.1.2 --- Treatments of MPS 1 --- p.4 / Chapter 1.2 --- Plant cells as bioreactors --- p.5 / Chapter 1.3 --- The Plant secretary pathway --- p.7 / Chapter 1.3.1 --- Transport of soluble proteins --- p.9 / Chapter 1.3.2 --- Transport of integral membrane proteins --- p.10 / Chapter 1.4 --- Differences between plant and human proteins --- p.11 / Chapter 1.5 --- Reducing the differences between plant and human proteins --- p.12 / Chapter 1.6 --- Previous study: Expression of IDUA in transgenic tobacco plant --- p.13 / Chapter 1.7 --- Project objectives --- p.14 / Chapter 1.8 --- Long term significance --- p.14 / Chapter Chapter 2 --- Materials and Methods --- p.15 / Chapter 2.1 --- Introduction --- p.16 / Chapter 2.2 --- Materials --- p.18 / Chapter 2.2.1 --- Chemical --- p.18 / Chapter 2.2.2 --- Plant materials --- p.18 / Chapter 2.2.3 --- Plasmid vectors and bacterial strains --- p.18 / Chapter 2.2.4 --- Human a-iduronidase (hIDUA) cDNA --- p.19 / Chapter 2.2.5 --- Primers --- p.20 / Chapter 2.3 --- Methods --- p.22 / Chapter 2.3.1 --- Generation of IDUA antibodies --- p.22 / Chapter 2.3.1.1 --- Synthetic peptide raised IDUA antibodies --- p.23 / Chapter 2.3.1.1.1 --- Design of synthetic peptides --- p.23 / Chapter 2.3.1.1.2 --- Immunization of rabbits --- p.25 / Chapter 2.3.1.2 --- E. coli-derived rhIDUA protein --- p.25 / Chapter 2.3.1.2.1 --- Cloning and expression of rhIDUA --- p.25 / Chapter 2.3.1.2.2 --- Western analysis of E. coli-derived rhIDUA --- p.29 / Chapter 2.3.1.2.3 --- MS/MS analysis of rhIDUA protein --- p.29 / Chapter 2.3.1.2.4 --- Immunization of rabbits --- p.31 / Chapter 2.3.2 --- Affinity-purified antibodies --- p.33 / Chapter 2.3.3 --- Characterization of affinity-purified IDUA antibodies --- p.33 / Chapter 2.3.4 --- Construction of chimeric gene constructs --- p.34 / Chapter 2.3.5 --- Expression of IDUA in tobacco BY-2 cells --- p.39 / Chapter 2.3.5.1 --- Electropoartion of Agrobacteria --- p.39 / Chapter 2.3.5.2 --- Agrobacterium-mediated transformation --- p.39 / Chapter 2.3.5.3 --- Screening of positive trans formants --- p.40 / Chapter 2.3.6 --- Characterization of transgenic BY-2 cell expressing IDUA fusion --- p.40 / Chapter 2.3.6.1 --- Genomic DNA polymerase chain reaction (Genomic DNA PCR) --- p.40 / Chapter 2.3.6.1.1 --- Genomic DNA extraction from BY-2 callus --- p.40 / Chapter 2.3.6.1.2 --- Genomic DNA PCR of tobacco BY-2 callus --- p.41 / Chapter 2.3.6.2 --- Reverse transcription-PCR (RT-PCR) --- p.42 / Chapter 2.3.6.2.1 --- Total RNA extraction from BY-2 cell --- p.42 / Chapter 2.3.6.2.2 --- RT-PCR of BY-2 cell --- p.42 / Chapter 2.3.6.3 --- Western blot analysis of BY-2 cell and medium --- p.43 / Chapter 2.3.6.3.1 --- Protein extraction from tobacco BY-2 cells and culture medium --- p.43 / Chapter 2.3.6.3.2 --- Sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) --- p.44 / Chapter 2.3.6.3.3 --- Immunodetection and Coomassie blue stain --- p.44 / Chapter 2.3.7 --- Purification of IDUA from culture media --- p.46 / Chapter Chapter 3 --- Results --- p.47 / Chapter 3.1 --- Generation of IDUA antibodies --- p.48 / Chapter 3.1.1 --- Cloning and expression of rhIDUA in E. coli --- p.48 / Chapter 3.1.2 --- Characterization of IDUA antibodies --- p.51 / Chapter 3.1.2.1 --- Specificity of IDUA antibodies towards hIDUA protein. --- p.51 / Chapter 3.1.2.2 --- Cross-reactivity of IDUA antibodies with wild type tobacco BY-2 cell --- p.55 / Chapter 3.2 --- Chimeric gene constructs construction and confirmation --- p.58 / Chapter 3.3 --- Screening of transformed tobacco BY-2 callus with kanamycin-resistance --- p.66 / Chapter 3.4 --- Genomic DNA PCR screening of transformed tobacco BY-2 callus . --- p.67 / Chapter 3.5 --- RT-PCR screening of transformed BY-2 cells --- p.70 / Chapter 3.6 --- Western blot analysis of transformed tobacco BY-2 cells and culture media --- p.72 / Chapter 3.6.1 --- Tobacco BY-2 cells --- p.72 / Chapter 3.6.2 --- Tobacco BY-2 cell culture media --- p.76 / Chapter 3.7 --- Purification of IDUA protein in culture media --- p.81 / Chapter Chapter 4 --- Discussion --- p.82 / Chapter Chapter 5 --- Summary and Future Perspectives --- p.89 / Chapter 5.1 --- Summary --- p.90 / Chapter 5.2 --- Future perspectives --- p.92 / Appendix Identification and Characterization of an Unknown Protein by 1B Antibody --- p.93 / Chapter 6.1 --- Introduction --- p.94 / Chapter 6.2 --- Objectives --- p.94 / Chapter 6.3 --- Materials and Methods --- p.95 / Chapter 6.3.1 --- Western blot analysis of different plant species --- p.95 / Chapter 6.3.2 --- Subcellular localization of the unknown protein --- p.95 / Chapter 6.3.3 --- Affinity-purification of the unknown protein --- p.95 / Chapter 6.4 --- Results --- p.97 / Chapter 6.4.1 --- Western blot analysis of different plant species --- p.97 / Chapter 6.4.2 --- Subcellular localization of an unknown protein --- p.98 / Chapter 6.4.3 --- Affinity-purification of 1B protein --- p.104 / Chapter 6.5 --- Summary and Future Perspectives --- p.105 / Chapter 6.5.1 --- Summary --- p.105 / Chapter 6.5.2 --- Future Perspectives --- p.105 / References --- p.106

Glycosidases--Synthesis

Tobacco--Cytology

Plant cell biotechnology

Transgenic plants

Iduronidase--biosynthesis

Lysosomes--enzymology

Tobacco--cytology

Plants, Genetically Modified

Amolecimento precoce da polpa e sua relação com as modificações da parede celular em mamões \'Golden\' / Flesh Early Softening in Golden papaya fruit and its relation to cell wall modifications

Gallon, Camilla Zanotti

01 March 2010

A ocorrência de mamões Golden com casca verde e polpa mole, em determinadas épocas do ano, tem sido relatada por produtores da região Norte do Espírito Santo. Não sendo possível distinguir frutos com o distúrbio do amolecimento precoce (DAP) apenas pela análise da cor da casca e da firmeza da polpa no momento da colheita, o objetivo deste trabalho foi estudar aspectos da fisiologia e bioquímica do amadurecimento que pudessem auxiliar no entendimento da perda precoce da firmeza. As coletas ocorreram no período de maior frequência de frutos com o distúrbio (meados de verão a final de outono). Os frutos foram coletados no estádio 1 de maturação, armazenados a 10º±1oC e 85±10% UR, durante 10 dias e submetidos à metodologia do Índice de Amolecimento (IA). O sintoma do amolecimento precoce foi observado claramente no 4°dia após o armazenamento sendo verificada a perda de firmeza nos frutos com DAP entre o 2° e o 8°dia a 10°C, sendo o decréscimo na firmeza equivalente a 71% da firmeza inicial, comportamento atípico para frutos armazenados sob refrigeração. Frutos com e sem DAP não apresentaram diferença significativa no teor de sólidos solúveis, acidez titulável e ácido ascórbico. A atividade respiratória e a produção de etileno foram reduzidas com o armazenamento refrigerado, sem diferença entre os frutos com e sem DAP, o que sugere que o aparecimento do distúrbio não se deve ao aumento na produção de etileno no período póscolheita. Os resultados indicam forte associação entre o amolecimento precoce e mudanças na parede celular. O rendimento das frações solúvel em água (FSA) e em NaOH (FSH) nos frutos com DAP, foi superior ao observado nos frutos sem DAP, durante todo o período de armazenamento. O menor nível da fração solúvel em imidazol (FSI) no tempo 0 pode estar associado à maior atividade da pectinametilesterase nos frutos com DAP. O decréscimo na fração celulose (CEL) em frutos com DAP pode indicar modificação na parede celular, ao nível celulose-hemicelulose. A produção de etileno não acompanhou as modificações na parede celular, sugerindo que alterações na estrutura da parede podem ter ocorrido durante o crescimento do fruto. Frutos com DAP apresentaram níveis de auxina (AIA) 6 vezes menor do que frutos sem DAP, no dia 0, sem diferença durante o armazenamento. Possivelmente os níveis de AIA nos frutos com DAP estavam reduzidos quando o fruto ainda estava ligado à planta. O distúrbio possivelmente está relacionado à alteração na parede celular e níveis de AIA. Desta forma, uma alteração hormonal durante o desenvolvimento do fruto anterior à colheita -, associada à sensibilidade do fruto à essa sinalização hormonal, levaria à mudanças na parede celular, o que determinaria a ocorrência do distúrbio do amolecimento precoce. / The occurrence of green skin and soft pulp in Golden papaya fruit during certain seasons has been reported by orchards in northern Espírito Santo State, Brazil. It is not possible solely by skin color and pulp firmness analysis to distinguish early softening disorder fruits (DAP), at the time of harvest, from those without the disorder. The aim of this work was to study the physiological and biochemical ripening aspects that might help to understand the early softening disorder. Fruits were harvested on the most common seasons (mid-summer to mid-autumn) in maturity stage 1 and evaluated for 10 days. Fruits were stored at 10°C, and submitted to softening index (IA). The symptoms of early softening disorder were clearly observed on the 4th day after storage. However, the firmness decrease in DAP fruits happened between the 2nd and 8th day at 10°C, with a decrease of 71% of initial firmness, presenting an atypical behavior for fruits stored under refrigeration. There was no difference between fruits with DAP and without DAP for soluble solids, titratable acidity and ascorbic acid content. Besides that, there was no difference between fruits with DAP and without DAP for respiration rate and ethylene production under refrigerated storage, which suggests that the disorder occurrence is not related to an increase in ethylene in the postharvest period. The results indicate a strong association between early softening disorder and changes in the cell wall composition. The cell wall polymers fractionation show that the yield of water soluble polymers (FSA) and NaOH soluble polymers (FSH) was higher in fruits with DAP than on fruits without DAP during the entire storage period. The smallest level of the imidazole soluble fraction (FSI) in DAP fruit, on day 0, may be related to a higher activity of pectinmethylesterase. The decrease in cellulose-rich polysaccharides (CEL) in the DAP fruit suggest modifications in the cellulose-hemicellulose domain. Ethylene production did not follow cell wall modification, suggesting that changes in the cell wall structure could be happening during fruit growth. DAP fruit presented an AIA level 6 times smaller than fruit without DAP, in day 0, without storage differences. Possibly, AIA levels in DAP fruit were reduced while fruits were still connected to the plant. The disorder may be related to cell wall changes and to AIA level. Should a hormonal change occur during fruit development i. e. prior to harvesting -- and still depending on fruit sensibility to hormonal signaling, cell wall changes could have different intensities, which determine if the fruit will or not have the flesh early softening observed after harvest.

Distúrbios fisiológicos de plantas

Enzimas

flesh.

Mamão

Maturação vegetal

maturation

papaya

Parede celular vegetal

Physiological disorder

plant cell wall

Polpa.